[Detailed Description of the Invention]
[Industrial Field of the Invention]
[0001] The present invention relates to a method for diluting a high viscosity liquid, and
more particularly to a method for diluting a red blood cell component of a blood sample,
which is employed in an apparatus for pipetting a blood sample.
[Prior Art]
[0002] Various kinds of tests are conducted on a blood sample collected from a human body.
For example, in a blood type test, as shown in Fig.10, a collected blood sample 10
is put into a test tube 12 and is then separated into a blood plasma component 14
and a red blood cell component 16 by centrifuging it or leaving it as it is. Practically,
a small quantity of white blood cell component 18 appears between the blood plasma
component 14 and the red blood cell component 16. Since the white blood cell component
18 is not relevant to the following description of the present invention, it is not
shown in other drawings.
[0003] A blood sample pipetting method which is carried out in a conventional pipetting
apparatus comprises two processes including a process of pipetting blood generally
plasma and a process of pipetting red blood cells. In the blood plasma pipetting process,
the blood plasma component 14 is aspirated through a nozzle tip 20, and then dispensed
into a plurality of other recipient containers 22 in a predetermined volume, respectively.
In the red blood cell pipetting process, the red blood cell component 16 is aspirated
through the nozzle tip 20, and then transferred to a diluting container (not shown)
to be mixed with a diluent. Thereafter, a diluted solution of red blood cell component
16 is aspirated again through the nozzle tip 20 and then dispensed into a plurality
of other recipient containers 24, respectively in a predetermined volume.
[0004] Blood type testing reagents (i.e., a reagent for the blood plasma component and a
reagent for the red blood cell component) are introduced into the recipient containers
22, 24, respectively.
[0005] Then, these recipient containers 22, 24 are conveyed to an agglutination testing
apparatus, where agglutination of the samples in the containers 22, 24 are measured
optically or visually. On the basis of the results of the measurements, A type, B
type, 0 type or AB type, or Rh type, or the like is determined.
[0006] Conventionally, dilution of the red blood cell component has been carried out in
the following manner. After having been aspirated by the nozzle tip, the red blood
cell component is first dispensed from the nozzle tip into the diluting container.
Before or after the dispensation of the red blood cell component, a predetermined
volume of diluent is introduced into the diluting container. The red blood cell component
is mixed and stirred with the diluent by blowing air into the container or vibrating
it. Thereafter, the diluted solution of the red blood cell component is aspirated
again through the nozzle tip, and then dispensed into the container 24.
[Problems to be solved by the Invention]
[0007] However, as well known, the red blood cell component is a high viscosity liquid (or
a gel-like substance), so it cannot be easily dispensed from the nozzle tip due to
its high viscosity. Consequently, quick dilution of the red blood cell component cannot
be achieved by the conventional diluting method.
[0008] In more detail, since the red blood cell component cannot be smoothly dispensed from
a smaller orifice in a distal end of the nozzle tip into the diluting container due
to its high viscosity, it takes a relatively long time to dispense the red blood cell
component into the diluting container. Consequently, in an apparatus for pipetting
a large volume of blood sample, it has been impossible to improve the pipetting ability.
[0009] For the above problems, it can be considered to enlarge the size of the smaller orifice
in the distal end of the nozzle tip. However, in that event, pipetting precision will
be lowered, and there will be caused an inconvenience of leakage or the like, when
transferring the liquid sample by using the nozzle tip. Consequently, a diluting method
for solving the above problems has been desired especially for a pipetting apparatus,
in which nozzle tips having the same shape are used to pipette the blood plasma component
and the red blood cell component.
[0010] This invention has been made in view of above problems.
[0011] It is therefore an object of the present invention to provide a method for diluting
as quickly as possible a high viscosity liquid sample, such as the red blood cell
component or the like.
[Means for Solving the Problems]
[0012] According to the present invention, the aforementioned object is achieved by a method
for diluting a high viscosity liquid, comprising the steps of aspirating a high viscosity
liquid sample by a nozzle tip, and mixing the liquid sample with a diluent, wherein
a distal end of the nozzle tip containing therein the liquid sample is inserted into
the diluent in a diluting container, aspiration is performed first, and then dispensation
and the aspiration are repeatedly performed.
[Operation of the Invention]
[0013] According to the aforementioned features of the present invention, the diluent is
first aspirated prior to dispensation of the high viscosity liquid sample from the
nozzle tip. After the liquid sample has been diluted to a certain degree, the mixed
liquid in the nozzle tip is dispensed. Further dispensation and aspiration are repeated.
Thus, it becomes possible to dilute the high viscosity liquid quickly.
[0014] Even if the nozzle tip contains the high viscosity liquid sample, it is easy to aspirate
and introduce the diluent into the high viscosity liquid sample in the nozzle tip,
as compared with the dispensation of the liquid sample. The dispensation of the red
blood cell component diluted to some degree with the diluent can be performed more
smoothly than dispensation of the pure red blood cell component. As a result, the
diluting time can be shortened, as compared with the conventional diluting method.
In the present invention, the first stage of the dilution takes place within the nozzle
tip.
[0015] It is preferable to increase the speed of the dispensing and aspirating operations
gradually in the mixing process in accordance with the degree of the dilution.
[Embodiments]
[0016] Embodiments of the present invention will now be described with reference to the
accompanying drawings.
[0017] Fig. 1 shows schematically a blood sample pipetting apparatus 30 (hereinafter called
"apparatus"), in which a high viscosity liquid diluting method of the present invention
is used. Fig. 1 is a perspective view of the apparatus 30.
[0018] In this embodiment, the apparatus 30 pipettes the blood plasma component and the
red blood cell component after centrifugation to perform a preprocess for blood type
test.
[0019] As shown substantially in the central portion of Fig. 1, a nozzle 32 for aspirating
a blood sample is held by an XYZ robot 34 so as to be movable three-dimensionally.
[0020] Fig. 2 shows a cross sectional view of a main part of the nozzle 32. The nozzle 32
is composed of a nozzle base 35, and a disposable tip serving as a nozzle tip 36.
Thus, the pipetting apparatus in the embodiment of the present invention uses a disposable
type nozzle tip. A distal end of the nozzle base 35 is forced into an upper opening
of the nozzle tip 36 and is fitted therein. Thus, the nozzle tip 36 is fixed firmly
to the nozzle base 35. The nozzle tip 36 has at its lower end a smaller orifice 36a
from which the blood sample is aspirated and dispensed. The nozzle tip 36 may be made
of a hard plastic material or the like, and the nozzle base 35 may be made of a metal.
[0021] In Fig. 1, the XYZ robot 34 is composed of an X drive portion 34x, an Y drive portion
34y and a Z drive portion 34z. To the Z drive portion 34z, an elevator 38 equipped
with the nozzle 32 is connected so as to be vertically movable. The elevator 38 has
a limit switch 40 serving as a jamming sensor or the like.
[0022] The limit switch 40 detects an external force imparted upwardly to the nozzle 32
and having a value greater than a predetermined force.
[0023] Onto the Z drive portion 34z, a diluent pipette 42 for dispensing a diluent is fixedly
mounted. An air hose 44 is connected at one end thereof to the nozzle 32 and at the
other end thereof to a syringe 46 serving as a pump for causing aspirating and dispensing
actions. A diluent hose 48 is connected at one end thereof to the diluent pipette
42 and at the other end thereof to a syringe 52 via an electromagnetic valve 50.
[0024] Between the syringe 46 and the nozzle 32, a pressure sensor 54 for measuring an internal
pressure of the air hose 44 is connected. A signal from the limit switch 40 is sent
to the apparatus via a cable 56.
[0025] On a test tube rack 60 placed on a pipetting table 58, a plurality of test tubes
62 containing blood samples which have been already subjected to a centrifugation
treatment are held uprightly. Each test tube 62, as shown in Fig. 10, contains the
blood sample in which the blood plasma component and the red blood cell component
are separated in an upper portion and a lower portion of the test tube 62, respectively.
On a horizontal table 64 mounted on the pipetting table 58, a dilution tray 68 provided
with a plurality of diluting containers 66, and a microplate 70 are provided. On the
microplate 70, a plurality of wells are provided for serving as a recipient container
for containing the blood plasma component or diluted solution of the red blood cell
component. After all of the blood samples have been pipetted, the microplate 70 is
conveyed to an apparatus of blood type test, by which an agglutination test, for example,
is made optically. The agglutination test may be made visually.
[0026] In the apparatus of the present invention, the nozzle tip is a disposable type and
is exchanged successively with a new one. A plurality of new nozzle tips are prepared
on a nozzle tip stand 72. There is also provided a nozzle scrap tray 74.
[0027] Therefore, in the apparatus of the present invention, it is possible that the blood
plasma component or the red blood cell component is aspirated by the nozzle tip 36
of the nozzle 32 and then transferred into other recipient container. The apparatus
may also be applied to purposes other than pipetting of the blood sample. Various
kinds of applications are possible.
[0028] Fig. 3 is a block diagram of the apparatus of the embodiment of the present invention.
By moving a piston 76 up and down, inside volume of the syringe 46 varies, so that
an aspirating pressure or a dispensing pressure is transmitted to the nozzle tip 36
of the nozzle 32 via the air hose 44 to perform aspiration or dispensation of the
blood sample. The internal pressure of the air hose 44 is detected by the pressure
sensor 54, a sensor signal outputted from the pressure sensor 54 is amplified by a
DC amplifier 78 and is then fed to an analog-digital converter 82 via a limiter circuit
80. The limiter circuit 80 is a protection circuit for suppressing any excessive input.
The analog-digital converter 82 converts the sensor signal into a digital signal and
feeds the digital signal to a control unit 84.
[0029] The control unit 84 includes a computer, for example, for controlling the inside
volume of the syringe 46 and the XYZ robot 34, etc. In the embodiment, the control
unit 84 also includes a viscosity measuring unit 86 and a table 88, both described
below.
[0030] Embodiments of a pipetting method of the present invention, used in the above-mentioned
apparatus will now be described below.
[0031] Figs. 4 and 5 show a blood plasma pipetting process. Fig. 4 shows a blood plasma
component aspirating process, and Fig. 5 shows a blood plasma component dispensing
step.
[0032] In Fig. 4, at step 101, the nozzle tip 36 is lowered from the upper side of the test
tube 62 and is stopped so that the distal end of the nozzle tip 36 is inserted into
the blood plasma component 90 to be positioned at a predetermined distance L1 downward
from a blood surface. L1 is preferably 2 to 3 mm. If the distal end of the nozzle
tip 36 is inserted too deeply into the blood plasma component 90, the two components
once separated by centrifugation are likely to be mixed again with each other.
[0033] When the nozzle tip 36 is lowered, the liquid surface is detected. This liquid surface
detection is performed by monitoring the internal pressure of the hose 44 by the pressure
sensor 54. When the internal pressure of the hose 44 is changed sharply, the control
unit 84 detects that the distal end of the nozzle tip 36 has reached the liquid surface.
[0034] At step 102, the blood plasma component 90 is aspirated. Specifically, the piston
76 is pulled downwardly to increase the inside volume of the syringe 46, whereby the
blood plasma is aspirated into the nozzle tip 36. For example, about 30 to 300 µl
of the blood plasma 90 is aspirated. As described in detail below, this aspirated
blood plasma component includes a small volume of blood plasma component to be used
for a plasma coating. Preferably, the volume of blood plasma component to be aspirated
should be determined by taking account of the volume of blood plasma component that
finally would attach onto an inner surface of the nozzle tip 36 and would not be dispensed
from the nozzle tip 36.
[0035] At step 103, the nozzle tip 36 is raised and stopped temporarily just before the
distal end of the nozzle tip 36 leaves from the liquid surface of the blood plasma
component 90. After a lapse of, for example, about 0.25 sec., the nozzle tip 36 is
raised again at step 104. The reason why the step 103 is needed in this process is
that the blood plasma component attaching onto an outer surface of the nozzle tip
36 is returned into the test tube 62, thereby improving the precision of the pipetting.
Next to step 104, step 105 of Fig. 5 is executed.
[0036] In the blood plasma dispensing process shown in Fig. 5, at step 105, the nozzle tip
36 is lowered into a predetermined well 92 and is stopped so that the distal end of
the nozzle tip 36 is positioned at a distance L2 off the bottom of the well 92. In
this case, L2 is preferably about 2 mm. If the blood plasma component is dispensed
from a too high position, it would become a drop, so that it is difficult to transfer
the blood plasma component into the well 92 quickly. Further, if the distal end of
the nozzle tip 36 comes into contact with the bottom of the well 92, it becomes very
difficult to dispense the blood plasma component.
[0037] For these reasons as stated in the above, preferable distance L2 is about 2mm in
view of the property of the liquid to be dispensed.
[0038] At step 106, a part (predetermined volume) of the blood plasma component existing
in the nozzle tip 36 is dispensed.
[0039] At step 107, the nozzle tip 36 is lowered until its distal end comes into slight
contact with the bottom of the well 92. The contact condition can be monitored by
the limit switch 40. At step 108, the nozzle tip 36 is raised. Namely, in step 107
and step 108, a so-called vertical touch-off system is employed, so that the blood
plasma component attaching onto the inner surface of the nozzle tip 36 can be dispensed
quickly.
[0040] At step 109, the nozzle tip 36 is raised and the same dispensing steps (S105-S109)
are repeated with respect to other wells. Finally, a predetermined volume of blood
plasma component is left in the nozzle tip 36, as shown at step 109 in Fig. 5. This
predetermined volume is preferably 15 to 20 µl. The final step 109 of the blood plasma
dispensing process shown in Fig. 5 corresponds to a coating preparing step, in which
a small volume of blood plasma component is left in the nozzle tip 36 for the purpose
of plasma coating.
[0041] Figs. 6 through 9 show the red blood cell pipetting process, which generally comprises
the following four processes including a blood plasma coating process of Fig. 6; a
red blood cell aspirating process of Fig. 7; a red blood cell diluting process of
Fig. 8; and a red blood cell diluted solution dispensing process of Fig. 9.
[0042] Firstly, the blood plasma coating process will now be described with reference to
Fig. 6. After step 109 of Fig. 5, step 200 of Fig. 6 is executed. Namely, by the XYZ
robot 34, the nozzle tip 36 is positioned above the test tube 62 from which the blood
plasma component has been aspirated at step 102. Specifically, the nozzle tip 36 is
positioned so that its distal end is inserted slightly (to be positioned at a distance
L3 off the blood surface) into the upper opening of the test tube 62. This positioning
would prevent the coating blood plasma from scattering over other blood samples and
contaminating them, thus improving the reliability of the apparatus. L3 at step 200
is preferably 5 mm.
[0043] In the method of this embodiment, pipetting operation is performed continuously by
using the same nozzle tip 36 throughout the blood plasma pipetting process and the
red blood cell pipetting process. Alternatively, when these two steps processes changeover,
the nozzle tip 36 may be exchanged with a new one. In such case, it is necessary to
provide a blood plasma component coating step as a preprocessing step before step
200.
[0044] At step 201, the blood plasma component used for the coating which remains in the
nozzle tip 36 is aspirated (raised) again at least to such an extent that the red
blood cell component to be subsequently aspirated reaches. Strictly, the inner surface
of tip 36 is coated to such an extent that the red blood cell component diluted later,
i.e., the diluted solution of red blood cells reaches.
[0045] At step 202, the blood plasma component for the coating is dispensed (lowered), and
the dispensation is stopped when the plasma component reaches the distal end of the
nozzle tip 36 as shown at step 203 of Fig. 6.
[0046] In this embodiment, the coating is accomplished by moving the blood plasma component
up and down only one time as shown at step 201 and step 202. Alternatively, the blood
plasma component may be moved up and down two or more times, if necessary. However,
it is confirmed that moving up and down one time is sufficient for the coating.
[0047] At step 204, the nozzle tip 36 is lowered and stopped when its distal end is inserted
into the blood plasma component 90 to be positioned at a distance L4 downward from
the blood surface. L4 is preferably 2 to 3 mm. At step 205, the remaining blood plasma
component used for the coating is returned into the test tube 62. Thus, in order to
use a valuable blood sample without wasting it, the blood plasma component for coating
is returned into the test tube 62. Although only a small volume of blood plasma component
is used for the coating in this embodiment, a large volume of blood plasma component
may be used for the coating. If a large volume of blood plasma component is used,
it is necessary to aspirate an unnecessarily large volume of blood plasma component
at step 102, and at step 205, when returning such large volume of blood plasma component
into the tube, there is a risk that the blood plasma component is mixed with the red
blood cell component. Consequently, it is preferable that the coating should be made
with a small volume of blood plasma component.
[0048] After step 205, step 206 of Fig. 7 is executed. At step 206, the nozzle tip 36 is
further lowered, so that its distal end is inserted into the red blood cell component
94. At that time, it is preferable that the distal end of the nozzle tip 36 is located
at a position of about 75% downward from the surface of the blood plasma component,
where the whole blood sample is 100%. If the nozzle tip 36 is inserted into the blood
plasma component too deeply, a large volume of red blood cell component 94 attaches
onto the outer surface of the nozzle tip 36. In contrast, if the nozzle tip 36 is
inserted into the blood plasma component too shallowly, it is difficult to aspirate
the red blood cell component surely.
[0049] At step 207, the red blood cell component 94 is aspirated. In this embodiment, for
example, 80 µl of red blood cell component 94 is aspirated.
[0050] However, the red blood cell component 94 is a high viscosity liquid or a gel substance,
so that considerable pressure and time are needed to aspirate such red blood cell
component via the smaller orifice of the distal end of the nozzle tip 36. In this
embodiment, the following two ways are used to improve the quickness of aspiration
to a maximum extent. In the first way, the inner surface of the nozzle tip 36 is coated
with the blood plasma component in order to reduce the frictional resistance of the
inner surface of the nozzle tip 36 as much as possible, thus ensuring a smooth aspiration
of the red blood cell component. In the second way, an excessively large volume of
red blood cell component is aspirated temporarily. Specifically, the piston 76 of
the syringe 46 is drawn to a maximum extent, and thereafter the internal pressure
of the air hose 44 is monitored by the pressure sensor 54. When the internal pressure
becomes equal to a predetermined value, the piston 76 is returned, so that only a
desired volume of red blood cell component is finally aspirated into the nozzle tip
36. That is, since a high viscosity solution of red blood cell component cannot be
aspirated so as to quickly follow the moving amount of the syringe 46, the maximum
aspiration force is applied to the nozzle 36, at an initial aspiration stage, the
moving amount of the syringe 46 is returned to a proper value just before a desired
volume of red blood cell component is aspirated, thereby obtaining a predetermined
volume of aspirated red blood cell component of which volume is to be determined by
the moving amount of the syringe 46. At step 208, when a detection value of the pressure
sensor 54 becomes substantially equal to an atmospheric pressure, the termination
of aspiration is confirmed. Strictly, since the red blood cell component is aspirated
into the nozzle tip 36, the internal pressure of the air hose 44 has a tendency to
become lower than the atmospheric pressure. Finally, at step 208, for example, 80
µl of the red blood cell component is aspirated into the nozzle tip 36.
[0051] At step 209, the nozzle tip 36 is raised slowly in order to keep the two blood components
stable in a separated state and in order to avoid causing any turbulent flow. Near
the liquid surface of the blood plasma component 90, the nozzle tip 36 is temporarily
stopped from raising as shown in step 209, and thereafter the nozzle tip 36 is raised
again at step 210.
[0052] At step 211, for example, about 10 µl of air is aspirated to provide an air cap 99
at the distal end of the nozzle tip 36. This enables to completely take in the nozzle
tip 36 the red blood cell component attaching to an edge of the distal end of the
nozzle tip 36, and to prevent the red blood cell component from dropping from the
nozzle tip 36.
[0053] The diluting process according to the present invention will now be described.
[0054] After step 211, step 212 of Fig. 8 is executed. In the step 212, the nozzle tip 36
is conveyed to an upper position above the diluting container 66, at which a predetermined
volume of diluent is dispensed into the diluting container 66 through the diluent
pipette 42. At step 213, the nozzle tip 36 is lowered from the upper position, so
that its distal end is positioned in the diluent 96 at a predetermined distance L5
off the bottom of the diluting container 66. L5 is preferably 2 mm. A physiological
salt solution can be used for the diluent.
[0055] At step 214, the diluent 96 is aspirated into the nozzle tip 36. In the conventional
method, the red blood cell component was dispensed to be mixed and diluted with the
diluent. However, in this embodiment, in view of the facts that the red blood cell
component is a high viscosity and dispensation thereof is relatively difficult, the
diluent which is easy to be aspirated is previously aspirated, and then the diluent
is mixed with the red blood cell component step by step.
[0056] At step 215, the mixed solution is dispensed from the nozzle tip 36 into the diluting
container 66. At that time, since the red blood cell component is previously diluted
by the diluent to a certain degree, the mixed solution can be dispensed extremely
easily, as compared with the dispensation of a pure red blood cell component. At step
216, the mixed solution, i.e., the diluted solution of red blood cell is aspirated.
In this embodiment, step 215 and step 216 are repeated about five times. During the
successive steps from step 214, the aspiration or dispensation is initially performed
slowly, depending on the viscosity of the substance to be aspirated or dispensed,
and thereafter progressively more quickly. At step 214, since the inner surface of
the nozzle tip 36 has been previously coated with the blood plasma component, the
diluent can be aspirated into the nozzle tip 36 more smoothly than the case in which
the inner surface of the nozzle tip 36 is not coated with the blood plasma component.
[0057] At step 217, the nozzle tip 36 is stopped temporarily from being raised when its
distal end reaches near the liquid surface, and then the nozzle tip 36 is raised again.
[0058] A process of dispensing the diluted solution of the red blood cell solution will
now be described.
[0059] After step 217, step 218 of Fig. 9 is executed. The nozzle tip 36 is conveyed to
a predetermined well 98 on the microplate by the XYZ robot. The nozzle tip 36 is lowered,
so that its distal end is positioned in the well 98 at a predetermined distance L6
downward from the upper opening of the diluting container 66, as shown at step 218.
L6 is preferably about 3 mm. Though there is not shown in the drawings, a predetermined
volume of reagent has been previously pipetted into the respective wells 98.
[0060] At step 219, a predetermined volume of diluted solution of red blood cell component
in the nozzle tip 36 is dispensed, and then a drop of the diluted solution formed
at the distal end of the nozzle tip 36 is attached onto the inner surface of the well
98 at step 220. Namely at step 220, by using the horizontal touch-off system, the
diluted solution of red blood cell component is dispensed, without bringing the distal
end of the nozzle tip 36 into direct contact with the reagent in the lower portion
of the well, thereby preventing contamination from being caused.
[0061] At step 221, the nozzle tip 36 is raised and then moved to a next well, and thereafter
the steps from step 218 to step 221 are repeatedly executed.
[0062] In this embodiment, after the blood plasma pipetting process and the red blood cell
pipetting process have been executed for a specific blood sample, the nozzle tip 36
is exchanged with a new one. By using this new nozzle tip, the blood plasma pipetting
process and the red blood cell pipetting process are executed in the same way for
other blood samples.
[0063] The viscosity measuring unit 86 of Fig. 3 will now be described hereinbelow. The
viscosity of the red blood cell component is valuable information for diagnosing an
illness and is also a valuable material for determining an aspiration pressure to
be set when a blood sample is pipetted. In the conventional apparatus, there is not
provided any viscosity measuring unit, and the viscosity of a blood sample is measured
by a separate measuring instrument. Therefore, after having been subjected to the
viscosity measurement, the blood sample has been disused. Further, the viscosity measurement
takes a long time and needs a complex operation.
[0064] In the apparatus of the present invention, since the control unit 84 is equipped
with the viscosity measuring unit 86, it is possible to measure the viscosity of the
blood sample while the blood sample being pipetted.
[0065] In various liquids having different viscosities, there is a close relationship between
the viscosity of each liquid and the time required from a point of time when a predetermined
pressure is produced as an initial aspiration pressure for aspirating the liquid to
a point of time when the aspiration pressure reaches a certain pressure value. It
was confirmed in a simulation that there is a proportional relation ship therebetween.
[0066] In a table 88, there is stored data which represents a relationship between the viscosity
of the liquid to be aspirated and the time required from a point of time when the
liquid begins to be aspirated under a certain initial aspiration pressure to a point
of time when the pressure which returns gradually to an atmospheric pressure reaches
a specifically set pressure value.
[0067] Specifically, when aspirating the blood sample into the nozzle tip 36, the internal
pressure of the air tube 44 is monitored by the pressure sensor 54, and the viscosity
measuring unit 86 measures the time required from a point of time when the piston
76 is drawn to give the initial aspiration pressure, to a point of time when the internal
pressure of the air tube 44 reaches a predetermined value. The viscosity measuring
unit 86 also obtains a viscosity of the blood sample by comparing the measured time
with the table 88. The obtained viscosity is indicated on a display unit (not shown),
and this result is utilized for controlling the syringe 46 by the control unit 84.
[0068] According to the viscosity measuring unit 86 described above, there are advantages
as follows. Since the viscosity can be measured simultaneously with the aspiration
of the blood sample, the unit 86 requires no additional time for measuring the viscosity,
and realizes a very simple viscosity measurement. Further, it is unnecessary to prepare
an additional blood sample only for viscosity measurement.
[Advantageous Effect of the Invention]
[0069] As explained in the above, in the mixing process of the present invention, the diluent
is aspirated before the red blood cell component is dispensed from the nozzle tip
into the diluting container. Thus, the dilution at a first stage is performed by using
the nozzle tip. Then, the diluted red blood cell component is repeatedly transferred
between the nozzle tip and the diluting container to perform dilution and mixing.
As a result, the method of the present invention makes it possible to dilute a high
viscosity liquid quickly, as compared with the conventional diluting method.
[0070] Therefore, the present invention has an advantage of improving the pipetting ability
when applied to an apparatus for pipetting a red blood cell component or the like.
[Brief Explanation of the Drawings]
[0071]
Fig. 1 is a schematic view for showing an embodiment of a pipetting apparatus in which
a diluting method of the present invention is used;
Fig. 2 is a cross-sectional view showing a main part of a nozzle;
Fig. 3 is a block diagram of the pipetting apparatus of Fig. 1;
Fig. 4 is an explanatory view for showing steps, in which blood plasma is aspirated
into the nozzle during a process of pipetting blood plasma;
Fig. 5 is an explanatory view for showing steps, in which the blood plasma is dispensed
from the nozzle during a process of pipetting the blood plasma;
Fig. 6 is an explanatory view for showing steps, in which the inner surface of the
nozzle is coated with the blood plasma during a process of pipetting red blood cells;
Fig. 7 is an explanatory view for showing steps, in which red blood cells are aspirated
into the nozzle during the process of pipetting the red blood cells;
Fig. 8 is an explanatory view for showing steps, in which the red blood cells are
diluted during the process of pipetting the red blood cells;
Fig. 9 is an explanatory view for showing steps, in which a red blood cell diluent
is dispensed from the nozzle during the process of pipetting the red blood cells;
and
Fig. 10 is an explanatory view for showing an operation of pipetting the blood plasma
and the red blood cells as a preprocess for a blood type test.
[Explanation of References Numerals]
[0072]
- 30
- pipetting apparatus
- 32
- nozzle
- 34
- XYZ robot
- 35
- nozzle base
- 36
- disposable tip
- 54
- pressure sensor
- 84
- control unit
- 86
- viscosity measuring unit
- 90
- blood plasma component
- 91
- red blood cell component